离体兔肝细胞质膜上内毒素脂多糖的结合位点。

Acta hepato-gastroenterologica Pub Date : 1979-10-01
G Ramadori, U Hopf, K H Meyer zum Büschenfelde
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引用次数: 0

摘要

采用免疫荧光技术研究了细菌脂多糖(LPS)在机械或酶分离兔肝细胞质膜上的体外固定。制备了兔抗大肠杆菌026:B6和0111:B4的血清。被动血凝试验测定抗体滴度高达1:1024。两种抗血清间无免疫交叉反应。从抗lps和正常兔血清中制备IgG和IgM,并与异硫氰酸荧光素偶联。针对LPS的抗体活性定位于IgM部分。采用无酶和胶原酶灌注法分离肝细胞。在0.01 ~ 1.0 mg / ml范围内,LPS与肝细胞质膜结合成正比增加,膜固定IgM抗LPS抗体在LPS包被的肝细胞表面呈粗颗粒状荧光。LPS与肝细胞的体外反应不受补体存在的影响。肝细胞质膜上LPS结合位点的发现支持了库普弗细胞和实质肝细胞参与肝脏内毒素清除活性的假设。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Binding sites for endotoxic lipopolysaccharide on the plasma membrane of isolated rabbit hepatocytes.

The in vitro fixation of bacterial lipopolysaccharide (LPS) on the plasma membrane of mechanically or enzymatically isolated hepatocytes from rabbits was studied by immunofluorescence technique. Antisera against LPS from E. coli 026:B6 and 0111:B4 were induced in rabbits. Antibody titers up to 1:1024 were determined by the passive hemagglutination test. There was no immunologic cross reactivity between the two antisera. IgG and IgM were prepared from anti-LPS as well as from normal rabbit serum and conjugated with fluorescein-isothiocyanate. The antibody activity against LPS was localized in the IgM fraction. Hepatocytes were isolated by a perfusion technique without enzymes and with collagenase. LPS binding to the hepatocellular plasma membrane increased proportionally with the LPS concentration in a range between 0.01 and 1.0 mg per ml. The fluorescence pattern of the membrane fixed IgM anti-LPS-antibody at the surface of LPS coated hepatocytes was coarse granular. The in vitro reaction of LPS with hepatocytes was not influenced by the presence of complement. The demonstration of binding sites for LPS on the hepatocellular plasma membrane supports the hypothesis that not only Kupffer cells but also parenchymal liver cells are involved in the hepatic clearance activity for endotoxin.

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